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  • Problem reading in fastq files in STAR

    Hi

    I am trying to read in my fastq files into STAR for mapping.
    My input data is organized as follows:
    1. 2 samples
    2. 3 replicates in each
    3. For each replicate, a number of paired end fastq files

    I have tried several methods to input but always get the error that could not open readInFile.

    For instance:
    Code:
    /home/STAR --genomeDir /media/ --readFilesIn /media/Sample1_R1_001.fastq /media/Sample1_R2_001.fastq,/media/Sample1_R1_002.fastq /media/Sample1_R2_002.fastq --runThreadN 4
    or
    Code:
    /home/STAR --genomeDir /media/ --readFilesIn /media/Sample1_R1_001.fastq Sample1_R2_001.fastq,Sample1_R1_002.fastq Sample1_R2_002.fastq --runThreadN 4
    Here, R1 and R2 are paired-end reads (separated by space). And Sample 1 has several such paired-end fastq files (i showed here 2 only just to be succint) (separated by ,). Similarly for other samples.

    Can anyone please suggest what might be going wrong?

    Thanks in advance.
    Best
    M

  • #2
    Try:
    Code:
    /home/STAR --genomeDir /media/ --readFilesIn /media/Sample1_R1_001.fastq,/media/Sample1_R1_002.fastq /media/Sample1_R1_001.fastq,/media/Sample1_R2_002.fastq --runThreadN 4
    Basically you need to separate the list of read #1 and read #2 files from each other by a space and separate different samples (or parts of a run) inside each of those by commas.
    Last edited by dpryan; 02-21-2014, 07:32 AM. Reason: Oops, I somehow created a "Sample3"! Mea culpa!

    Comment


    • #3
      Hi dpryan

      Thanks for your input.
      What you have suggested is what I am doing but it is not working.
      As I mentioned previously,
      Sample 1 has paired-end reads (R1 and R2) which are present as 15 fastq files (i.e. Sample1_R1_i and Sample1_R2_i, where i=1-15).
      Similarly I have multiple paired-end files for other samples.

      As you suggested,
      Code:
      separate the list of read #1 and read #2 files from each other by a space
      that would mean separating R1 and R2 by a space

      Code:
      separate different samples (or parts of a run) inside each of those by commas
      that would mean separating R1_1 and R1_2 by ,.

      This would translate to (showing it for 3 paired-fastq files only for sample1)
      Code:
      /home/STAR --genomeDir /media --readFilesIn /media/Sample1_R1_001.fastq /media/Sample1_R2_001.fastq,/media/Sample1_R1_002.fastq /media/Sample1_R2_002.fastq,/media/Sample1_R1_003.fastq /media/Sample1_R2_003.fastq --runThreadN 4
      I have also tried listing all the R1 reads (separated by ,) followed by a space and then listing all R2 reads (separated by ,) butthat also doesnot work.

      On a similar note, should I run mapping for my other samples in the same command or issue a fresh command?

      Thanks.
      Best
      M

      Comment


      • #4
        No, for a list of 3 that would mean:

        Code:
        /home/STAR --genomeDir /media --readFilesIn /media/Sample1_R1_001.fastq,/media/Sample1_R1_002.fastq,/media/Sample1_R1_003.fastq /media/Sample1_R2_001.fastq,/media/Sample1_R2_002.fastq,/media/Sample1_R2_003.fastq --runThreadN 4
        The general idea is "R1_1,R1_2,R1_3,R1_4,...,R1_N R2_1,R2_2,R2_3,R2_4,...,R2_N".

        Comment


        • #5
          Ok. Got it.
          Its working now.
          And should I include other samples also (Sample2, 3 etc) also in the same command or give individual separate commands for each of them.

          Thanks.
          M

          Comment


          • #6
            Since it outputs to a single file (at least if memory serves me correctly), run them separately so you can get each sample in a different file.

            BTW, one trick is to load the genome into memory once and then only remove it when you're done. This is easiest if you're running things in a script that iterates through samples (this is the approach I take on our cluster).

            Comment

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